Beruflich Dokumente
Kultur Dokumente
Asian Journal of
Food and Agro-Industry
ISSN 1906-3040
Available online at www.ajofai.info
Research Article
Abstract
Milk and milk products have been considered to be an important nutritional food because they
are good sources of protein and calcium. However, most people have suffered from
gastrointestinal problems such as bloating, nausea, gas and diarrhea after drinking milk and
milk products as called lactose intolerance. This is due to the inability to digest the lactose
which is a major sugar found in milk. It is thus desirable to remove lactose from milk to
accommodate people suffered from lactose intolerance and to improve its storage stability and
functionality. Ultrafiltration (UF) is an attractive process for reducing lactose from dairy
products because it has MWCO in the range of 1,000-500,000 Dalton. Therefore, lactose can
easily pass through the membrane while retain all the protein in the retentate. Even though
other minerals such as calcium can also pass through the membrane, they can be recovered by
heating and adjusting the pH of the permeate. The separated lactose in the permeate can be
used for functional foods production such as galacto-oligosaccharides which can be
supplemented into the low lactose products or other dairy products. The goal of this project is
to evaluate the feasibility of removing lactose from milk by UF and to determine effects of
transmembrane pressure and feed flowrate on permeate flux and rejections of protein and
lactose. A Quixstand Benchtop cross flow hollow-fiber system is used in this project. UF
membrane with MWCO of 5,000 Dalton is selected for lactose separation. The effects of
transmembrane pressure and feed flow rate on lactose and protein rejection, lactose recovery
yield and permeate flux were evaluated. Our results showed that the lactose and protein
rejection value were approximately 13% and 100% respectively. A high degree of removal of
lactose from milk could be achieved. Therefore, the low lactose milk and milk products can
be obtained by this technique.
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Keywords: dairy, ultrafiltration membrane, low lactose milk, hollow fibre, galactooligosaccharides, Thailand
Introduction
Milk and milk products have been considered to be an important nutritional food because they
are good sources of protein, vitamins and calcium. However, many people suffer from lactose
intolerance making them unable to consume milk and dairy-based products. This is due to the
inability to digest the lactose which is a major sugar found in milk. The maldigestion of
lactose can cause the gastrointestinal problems such as bloating, nausea, gas and diarrhea.
Therefore, it is desirable to remove lactose from milk to minimize lactose maldigestion. In
general, there are several technologies for removing lactose from milk. Lactose can be
hydrolyzed into glucose and galactose. This method, however, has some disadvantages in
terms of sweetness. It has been reported that the sweetness increases up to 70% related to
sucrose [1]. This can be advantage or disadvantage depending on the purpose of the products.
The removal of lactose can also improve its solubility, storage stability, and functionality [1,
2]. Another approach to separate lactose is crystallization. This method, however, is limited to
by products from whey or whey permeate [2]. Recently, membrane technology has gained
more interest because of its energy saving process. Ultrafiltration membranes (UF) have
molecular weight cut-off in the range of 1,000-500,000 Daltons [3]. Therefore, lactose can
easily pass through the membrane while retain all fat and milk proteins in the retentate. Even
though other nutritional minerals such as calcium can also pass through the membrane, they
can be recovered by heating and adjusting the pH of the permeate [2]. The separated lactose in
the permeate can be used for functional foods production such as galacto-oligosaccharides
which can be supplemented back into the low lactose products or other dairy products [4, 5,
6]. The milk retentate from ultrafiltration is considered to be concentrated milk which is
suitable for cheese and yoghurt production [5, 7]. The objective of this work was to determine
effects of process parameters (transmembrane pressure and feed flow rate) on permeate flux
and rejections of protein and lactose.
Materials and Methods
Commercial low-fat UHT milk under the brand name of Foremost was used as raw material
in all experiments. The following parameters were measured: protein (Bradford Biorad Assay
kit), lactose (HPLC) and permeate flux.
Filtration system
A cross-flow hollow fibre unit (Quixstand- Benchtop system, GE Healthcare Bioscience,
USA) was used for the laboratory scale ultrafiltration experiments. Figure 1 shows the
schematic diagram of this cross-flow separation unit. A commercial hollow-fibre cartridge
membrane from Amersham (GE Healthcare Bio-science, USA) with a molecular weight cutoff 5,000 Dalton was used in this study. The membrane effective surface area is 650 cm2. Pure
water flux (PWF) was measured before each run in order to test whether the membrane was
damaged. The acceptable fluctuation range for an undamaged membrane is within 20%.
Permeate and retentate solutions were collected to measure lactose concentrations by HPLC.
After each run, the membrane was rinsed and cleaned in situ with distilled water followed by
0.1 N NaOH for 30 mins, thoroughly drained the system and rinsed the cartridge with distilled
water until the pH is neutral. PWF after cleaning was also measured to determine whether the
membrane was clogged or fouled.
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BackpressureValve
Diafiltration line
Recirculation
reservoir
Sampling/ Drain
valve
Peristaltic
Pump
Inlet pressure
Gauge
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(2)
where Cr and Cf are retentate and feed concentration, respectively. The equation for volume
concentration factor (VCF) is given by
(3)
where Vf and Vr are the feed and retentate volume, respectively.
The % recovery of lactose in permeate is calculated from the fraction of lactose in the
permeate recovered from the original feed.
(4)
where Cp and Vp are permeate concentration and permeate volume, respectively.
Results and Discussion
Effects of transmembrane pressure
Pressure is the main driving force in the membrane separation process. The effects of the
transmembrane pressure on permeate flux and rejections of lactose and protein were thus
studied. Figure 2 presents the permeate flux at different transmembrane pressure while the
feed flow rate was maintained constant at 0.64 L/min. In general, there was a linear
correlation between the transmembrane pressure difference and the permeate flux up to 4.5
psig. Beyond 4.5 psig, there was no significant increase in the permeate flux, indicating that it
reached the limiting flux, J as the resistance in the membrane boundary layer also increased
with increasing the pressure [3,8]. The effect of transmembrane pressure on %lactose
recovery is shown in Figure 3. As can be seen, % lactose recovery had the same correlation
with the permeate flux. At pressure beyond 4.5 psig, % lactose recovery decreased indicating
the concentration polarization problem occurred on the membrane surface. Table 1 shows the
effects of transmembrane pressure on lactose and protein rejections. There was no protein lost
in the permeate. Therefore, the transmembrane pressure of 4.5 psig was selected to be the
operating pressures for this application because it gave a high permeate flux without reaching
the limiting flux region. Also, the amount of lactose recovered in the permeate was
significantly high at this transmembrane pressure.
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Figure 2. Effect of transmembrane pressure on permeate flux with a constant feed flow rate at
0.64 L/min.
% rejection
lactose
protein
48.7
99.7
22.1
100
20.0
100
13.1
100
15.5
100
241
242
lactose
30.2
18.2
11.3
12.2
% rejection
protein
99.9
99.7
99.8
100
Conclusion
Both transmembrane pressure and feed flow rate affected the permeate flux, lactose rejection
and % lactose recovery. A high degree of removal of lactose from milk could be achieved by
UF with a minimal or no lost of protein in the permeate. Therefore, the low lactose milk and
milk products can be obtained by this technique and the separated lactose can be used as
substrates for functional food production.
Acknowledgment
This work was financially supported by the Faculty of Engineering and Industrial
Technology, Silpakorn University.
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